Distribution of viral antigen gp85 and provirus in various tissues from commercial meat-type and experimental White Leghorn Line 0 chickens with different subgroup J avian leukosis virus infection profiles

Distribution of viral antigen gp85 and provirus in various tissues from commercial meat-type and experimental White Leghorn Line 0 chickens with different subgroup J avian leukosis virus infection profiles

Immunohistochemistry and polymerase chain reaction (PCR) were used to test for the presence of avian leukosis virus (ALV) J viral antigen gp85 and proviral DNA, respectively, in various tissues (adrenal gland, bone marrow, gonad, heart, kidney, liver, lung, pancreas, proventriculus, sciatic nerve, s...

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Veröffentlicht in:Avian pathology 2008-02, Vol.37 (1), p.7-13
Hauptverfasser: Pandiri, A.R, Gimeno, I.M, Reed, W.M, Lee, L.F, Silva, R.F, Fadly, A.M
Format: Artikel
Sprache:eng
Schlagworte:
accuracy
animal age
animal tissues
Animals
antibodies
Antigens
Antigens, Viral - isolation & purification
Antigens, Viral - metabolism
Avian Leukosis - metabolism
Avian Leukosis - virology
Avian leukosis virus
Avian Leukosis Virus - classification
broiler chickens
Chickens - genetics
diagnostic techniques
DNA, Viral - isolation & purification
glycoproteins
immunohistochemistry
Infections
Meat
microbial genetics
molecular sequence data
neutralizing antibodies
nucleotide sequences
polymerase chain reaction
Poultry
poultry diseases
proviruses
Proviruses - isolation & purification
Retrospective Studies
seroconversion
temporal variation
test sensitivity
Tissues
vertebrate viruses
viral antigens
Viruses
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Zusammenfassung:Immunohistochemistry and polymerase chain reaction (PCR) were used to test for the presence of avian leukosis virus (ALV) J viral antigen gp85 and proviral DNA, respectively, in various tissues (adrenal gland, bone marrow, gonad, heart, kidney, liver, lung, pancreas, proventriculus, sciatic nerve, spleen, and thymus). Tissues were collected from 32-week-old commercial meat-type and Avian Disease and Oncology Laboratory experimental White Leghorn Line 0 chickens with the following different infection profiles: tV + A−, included in ovo-tolerized viraemic chickens with no neutralizing antibodies (NAbs) on any sampling; ntV + A−, included chickens that were viraemic and NAb-negative at the time of termination at 32 weeks post hatch, but had NAbs on up to two occasions; V+ A+, included chickens that were viraemic and NAb-positive at the time of termination at 32 weeks post hatch, and had NAbs on more than two occasions; V − A+, included chickens that were negative for viraemia and NAb-positive at the time of termination at 32 weeks post hatch, and had antibody on more than two occasions; V − A−, included chickens that were never exposed to ALV J virus. There was a direct correlation between viraemia and tissue distribution of gp85, regardless of the NAb status and strain of chickens, as expression of ALV J gp85 was noted in only viraemic chickens (tV + A−, ntV + A−, V+ A+), but not in non-viraemic seroconverted chickens (V − A+). Of the four oligonucleotide primers pairs used in PCR to identify ALV J provirus, only one primer set termed H5/H7 was useful in demonstrating ALV J proviral DNA in the majority of the tissues tested from non-viraemic, antibody-positive chickens (V − A+). The results suggest that PCR using primer pair H5/H7 is more sensitive than immunohistochemistry in identifying ALV J in chickens that have been exposed to virus, but are not actively viraemic.
ISSN:0307-9457
1465-3338
DOI:10.1080/03079450701774843